TO THE EDITOR: In a recent issue of The Journal Nuclear Medicine, 2 interesting papers on PET detection of epidermal growth factor receptor (EGFR) in cancer were published (1,2). Liu et al. reported the potential of 11C-PD153035 for the imaging of EGFR expression in humans, especially in non–small cell lung cancer (1). Tolmachev et al. reported that radiometal-labeled monomeric ZEGFR:1907 is the preferable format of EGFR-specific Affibody (Affibody AB) for imaging EGFR expression in mice with A431 cervical carcinoma xenografts (2).
The 2 articles differ from each other in several ways, such as the setting (humans and animals, respectively), the approach (labeled tyrosine kinase [TK] inhibitors and monoclonal antibody anti-EGFR, respectively), and the aims (metabolism/radiation dosimetry and imaging potential, respectively). Despite these relevant differences, both articles highlight an important issue for nuclear medicine and medical oncology research. The problem of detecting in vivo EGFR with a noninvasive approach is one of the most challenging in the selection of patients to receive EGFR inhibitors. However, some areas of discussion in these 2 papers need to be examined.
In brief, Lu et al. chose PD153035, a small-molecule TK inhibitor, labeled with 11C as a promising PET tracer. PD153035 is a reversible EGFR inhibitor and has been considered the prototype of this class of tracer (3,4). However, a preclinical study performed on tumor-bearing nude mice showed that the reversible compound may have a high non–tumor-specific uptake, probably bringing about a high competition with intracellular adenosine triphosphate at the binding site of the compound (5). However, the reason this study is of great interest is because it was the first such study performed on humans and opened the possibility of further clinical investigations. In Western countries, this aspect is relevant because the legislative process before a pharmaceutical drug can first be investigated in humans is lengthy and requires great effort. As a consequence, some promising novel tracers for EGFR imaging investigated in the United States or Europe still face extensive delays before being translated into human studies.
Tolmachev et al. chose the totally different approach of labeling the monoclonal antibody anti-EGFR. The strength of their study is that they used an Affibody that has a molecular weight lower than that of monoclonal antibodies, permitting high-contrast images of tumor receptor expression. The same approach had already shown successful results for HER2 imaging (6). However, some doubts still remain on the possibility of using it for imaging liver metastases or for metastatic sites near the kidneys.
During the last few years, several papers have been published on this topic and several advances have been made, but we believe that the development of the ideal PET tracer for EGFR imaging is still far distant (7–9). From an oncologic point of view, we need to discuss the actual usefulness of in vivo detection of EGFR expression in cancer today. As is well known, the most reliable clinical application is the prediction of anti-EGFR treatment response. However, during the last few years, advances in molecular predictive factors have been made. After the first evidence had been found by Lynch et al. and Paez et al. (10,11), several papers showed that EGFR mutational status is a sensitive predictor of TK inhibitor activity in lung cancer. Furthermore, K-ras mutational status now represents the main available biomarker discriminating responders from nonresponders to anti-EGFR monoclonal antibodies in colorectal cancer and is the only one that should be translated into everyday clinical practice (12). Anti-EGFR drugs showed activity independently of total EGFR quantity; consequently, interest in the detection of receptor expression was lost. Moreover, we can suppose that the difficulties that emerged for EGFR imaging depended on the receptor amount, which was probably much too low to be detected in vivo. The approach of in vivo molecular imaging of membrane receptors may be more feasible and useful only in cases of receptor amplification, such as HER2 in breast cancer. As a consequence, we should pay more attention to both the activation of the receptor and its downstream signaling pathway, which are, respectively, influenced by EGFR and K-ras gene mutations. In fact, Pal et al. showed that the activation status of EGFR may be detected by in vivo imaging using PET probes that specifically bind only the adenosine triphosphate site of phosphorylated EGFR TK (13). Memon et al. showed that nude mice bearing xenografts of HCC827 cells harboring an in-frame deletion-mutation in exon 19 had the highest uptake of 11C-erlotinib (14). In both studies, the specific use of activated or mutated cell lines for the development of the animal model suggested that EGFR PET may be strictly dependent on the functional and mutational status of the receptor. Moreover, it was reported that the biologic features underlying the various EGFR mutations in non–small cell lung cancer are distinct and thus may confer different cellular properties or different TK activities and, consequently, different sensitivities to EGFR inhibitors (15). This variability should also be considered in the development of animal models and the design of chemical compounds as PET probes.
Currently, the added value of studying and using PET tracers for EGFR in clinical practice would be the possibility of obtaining information in vivo, in contrast to ex vivo molecular techniques, and of obtaining global information on all metastatic sites and with a repeatable approach during the progression of disease (16). Nevertheless, we would like to underline that the truly useful information is related to the cellular functional modifications underlying EGFR activation and not to EGFR expression.
In conclusion, over the near term, it would be more challenging to focus on imaging receptor function, which one can influence by mutations or by an aberrant downstream signaling pathway in order to reflect the complexity and variability of the EGFR pathway in human cancer. At any rate, the recent papers and all ongoing projects contribute to improving our understanding of this fascinating but also extremely difficult facet of nuclear medicine and medical oncology.
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